Markers of definitive endoderm

a technology of endoderm cells and markers, which is applied in the field of cell biology and medicine, can solve the problems of limited islet cell donor pancreases, unique challenges, and inability to generate insulin-producing -cells from hescs, and achieve the effect of promoting the differentiation of said pluripotent cells

Active Publication Date: 2013-11-19
VIACYTE INC
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Benefits of technology

[0008]In certain embodiments, the method of producing a cell population enriched for definitive endoderm cells can also include the following steps: obtaining a cell population comprising pluripotent human cells; providing the cell population with at least one growth factor of the TGFβ superfamily in an amount sufficient to promote differentiation of said pluripotent cells to definitive endoderm cells; and allowing sufficient time for definitive endoderm cells to form. In further embodiments, the at least one growth factor can be selected from the following: Nodal, activin A, activin B and combinations thereof. In some embodiments, the at least one growth factor can be provided to said cell population at a concentration ranging from about 1 ng / ml to about 1000 ng / ml. In further preferred embodiments, the at least one growth factor can be provided in a concentration of at least about 100 ng / ml. In other preferred embodiments, the cell population can be grown in a medium including less than about 10% serum. In yet other preferred embodiments, the pluripotent human cells can be human embryonic stem cells.
[0010]In some embodiments, the step of differentiating the pluripotent cells can include providing the cell population with at least one growth factor of the TGFβ superfamily in an amount sufficient to promote differentiation of said pluripotent cells to definitive endoderm cells, and allowing sufficient time for definitive endoderm cells to form. For example, in some embodiments, the cell population can be provided with at least one growth factor selected from the group consisting of Nodal, activin A, activin B and combinations thereof. In preferred embodiments, the at least one growth factor can be provided to said cell population at a concentration ranging from about 1 ng / ml to about 1000 ng / ml. In other preferred embodiments, the at least one growth factor can be provided in a concentration of at least about 100 ng / ml. In still other preferred embodiments, the cell population can be grown in a medium including less than about 10% serum. In yet other preferred embodiments, the pluripotent human cells can be human embryonic stem cells.

Problems solved by technology

However, presently it is not known how to generate an insulin-producing β-cell from hESCs.
As such, current cell therapy treatments for diabetes mellitus, which utilize islet cells from donor pancreases, are limited by the scarcity of high quality islet cells needed for transplant.
Although pluripotency imparts extraordinary utility upon hESCs, this property also poses unique challenges for the study and manipulation of these cells and their derivatives.

Method used

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Examples

Experimental program
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example 1

Human ES Cells

[0255]For our studies of endoderm development we employed human embryonic stem cells, which are pluripotent and can divide seemingly indefinitely in culture while maintaining a normal karyotype. ES cells were derived from the 5-day-old embryo inner cell mass using either immunological or mechanical methods for isolation. In particular, the human embryonic stem cell line hESCyt-25 was derived from a supernumerary frozen embryo from an in vitro fertilization cycle following informed consent by the patient. Upon thawing the hatched blastocyst was plated on mouse embryonic fibroblasts (MEF), in ES medium (DMEM, 20% FBS, non essential amino acids, beta-mercaptoethanol, and FGF2). The embryo adhered to the culture dish and after approximately two weeks, regions of undifferentiated hESCs were transferred to new dishes with MEFs. Transfer was accomplished with mechanical cutting and a brief digestion with dispase, followed by mechanical removal of the cell clusters, washing an...

example 2

hESCyt-25 Characterization

[0257]The human embryonic stem cell line, hESCyt-25 has maintained a normal morphology, karyotype, growth and self-renewal properties over 18 months in culture. This cell line displays strong immunoreactivity for the OCT4, SSEA-4 and TRA-1-60 antigens, all of which, are characteristic of undifferentiated hESCs and displays alkaline phosphatase activity as well as a morphology identical to other established HESC lines. Furthermore, the human stem cell line, hESCyt-25, also readily forms embryoid bodies (EBs) when cultured in suspension. As a demonstration of its pluripotent nature, hESCyT-25 differentiates into various cell types that represent the three principal germ layers. Ectoderm production was demonstrated by Q-PCR for ZIC1 as well as immunocytochemistry (ICC) for nestin and more mature neuronal markers. Immunocytochemical staining for β-III tubulin was observed in clusters of elongated cells, characteristic of early neurons. Previously, we treated EB...

example 3

Production of SOX17 Antibody

[0258]A primary obstacle to the identification of definitive endoderm in hESC cultures is the lack of appropriate tools. We therefore undertook the production of an antibody raised against human SOX17 protein.

[0259]The marker SOX17 is expressed throughout the definitive endoderm as it forms during gastrulation and its expression is maintained in the gut tube (although levels of expression vary along the A-P axis) until around the onset of organogenesis. SOX17 is also expressed in a subset of extra-embryonic endoderm cells. No expression of this protein has been observed in mesoderm or ectoderm. It has now been discovered that SOX17 is an appropriate marker for the definitive endoderm lineage when used in conjunction with markers to exclude extra-embryonic lineages.

[0260]As described in detail herein, the SOX17 antibody was utilized to specifically examine effects of various treatments and differentiation procedures aimed at the production of SOX17 positiv...

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Abstract

Disclosed herein are reagent-cell complexes comprising one or more definitive endoderm cells. Also described herein are compositions for detecting definitive endoderm. Method of enriching, isolating and / or purifying definitive endoderm cells are also disclosed.

Description

RELATED APPLICATIONS[0001]This application is a U.S. national phase application under 35 U.S.C. §371 of International Application No. PCT / US2006 / 043932, entitled MARKERS OF DEFINITIVE ENDODERM, filed Nov. 13, 2006, designating the United States and published in English on May 24, 2007 as WO2007 / 059007, which is a nonprovisional application claiming priority under 35 U.S.C. §119(e) to U.S. Provisional Patent Application No. 60 / 736,598, entitled MARKERS OF DEFINITIVE ENDODERM, filed Nov. 14, 2005; this application is also a continuation-in-part of U.S. patent application Ser. No. 11 / 021,618, entitled DEFINITIVE ENDODERM, filed Dec. 23, 2004, which claims priority under 35 U.S.C. §119(e) as a nonprovisional application to U.S. Provisional Patent Application No. 60 / 587,942, entitled CHEMOKINE CELL SURFACE RECEPTOR FOR THE ISOLATION OF DEFINITIVE ENDODERM, filed Jul. 14, 2004; and U.S. Provisional Patent Application No. 60 / 586,566, entitled CHEMOKINE CELL SURFACE RECEPTOR FOR THE ISOLATI...

Claims

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Application Information

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Patent Type & Authority Patents(United States)
IPC IPC(8): C12N5/00C12N5/073
CPCC12N5/0603C12N5/0617C12N2501/16A61K35/38A61K35/407C12N5/0672C12N5/068C12N2501/415
Inventor D'AMOUR, KEVIN ALLENAGULNICK, ALAN DBAETGE, EMMANUEL EDWARD
Owner VIACYTE INC
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